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Báo cáo y học: "The first report of human illness associated with the Panola Mountain Ehrlichia species: a case report" doc

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BioMed Central Page 1 of 3 (page number not for citation purposes) Journal of Medical Case Reports Open Access Case report The first report of human illness associated with the Panola Mountain Ehrlichia species: a case report Will K Reeves* 1,3 , Amanda D Loftis 2,3 , William L Nicholson 3 and Alan G Czarkowski 3 Address: 1 USDA-ARS-ABADRL, Department 3354, 1000 E University Ave, Laramie, WY 82071-2000, USA, 2 226 North Lincoln St, Laramie, WY 82070, USA and 3 Centers for Disease Control and Prevention, 1600 Clifton Rd NE, MS G-13, Atlanta, GA 30333, USA Email: Will K Reeves* - will.reeves@ars.usda.gov; Amanda D Loftis - adloftis@gmail.com; William L Nicholson - wln4@cdc.gov; Alan G Czarkowski - bkt3@cdc.gov * Corresponding author Abstract Introduction: Two species of Ehrlichia are known to cause human illness. Several other species have been discovered in ticks and animals, and recent reports suggest that some of these Ehrlichia species might be human pathogens. We report here the first association of a recently discovered pathogen, the Panola Mountain Ehrlichia species, with a case of human illness. Case presentation: A 31-year-old man from Atlanta, Georgia (GA) in the United States of America (USA) presented with a persistent sore neck of 3 weeks duration following a tick bite. DNA from the Panola Mountain Ehrlichia species, which was recently discovered in a goat in Georgia, was detected in an acute blood sample. Serologic testing was inconclusive. Polymerase chain reaction tests for other tick-borne diseases found in this region were negative. The patient rapidly improved in response to doxycycline therapy. Conclusion: Detection of Ehrlichia DNA in an acute blood sample meets the Centers for Disease Control and Prevention laboratory confirmation criteria for ehrlichiosis, and response to doxycycline provides supporting clinical evidence. The Panola Mountain Ehrlichia species, an emerging pathogen transmitted by ticks in the eastern USA, should be considered as a possible cause of tick-borne illness in this region. Introduction Ehrlichia species are tick-transmitted intracellular bacteria closely related to Anaplasma, Neorickettsia and Rickettsia. Ehrlichia chaffeensis was first described as a human patho- gen in 1986 and E. ewingii in 1996 [1], and recent evi- dence suggests that other species of Ehrlichia might also cause illness [2,3]. A new species of Ehrlichia, the Panola Mountain Ehrlichia species, was recently discovered in the USA [4]. Clinical signs of ehrlichial infection are often non-specific, and the most common signs are fever, head- ache, myalgia and malaise [1]. Laboratory diagnosis of ehrlichiosis depends on the detection of ehrlichiae in samples collected during the acute illness or on demon- stration of a significant rise (four-fold or greater) in anti- body titer between the acute and convalescent phases of the illness [1,5]. Serology is limited because acute serol- ogy alone is insufficient to diagnose infection, paired serology does not provide a diagnosis until 3 to 4 weeks Published: 30 April 2008 Journal of Medical Case Reports 2008, 2:139 doi:10.1186/1752-1947-2-139 Received: 31 December 2007 Accepted: 30 April 2008 This article is available from: http://www.jmedicalcasereports.com/content/2/1/139 © 2008 Reeves et al; licensee BioMed Central Ltd. This is an Open Access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/2.0 ), which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited. Journal of Medical Case Reports 2008, 2:139 http://www.jmedicalcasereports.com/content/2/1/139 Page 2 of 3 (page number not for citation purposes) after empirical treatment has been initiated, and only E. chaffeensis is available for serologic testing of humans [1]. Diagnosis of ehrlichiosis during the acute infection increasingly relies on polymerase chain reaction (PCR) [1,6]. According to the official case definition used by the Centers for Disease Control (CDC) and the USA National Notifiable Diseases System, a positive PCR reaction, with confirmation of the amplicon identity, is sufficient for laboratory confirmation of a case of human ehrlichiosis [5]. Case presentation On 23 September 2005, a 31-year-old Caucasian man from Atlanta, Georgia, USA presented with a complaint of neck soreness for 3 weeks. The patient reported hiking at Panola Mountain State Park in Georgia on 31 August 2005 and later removing a partially engorged nymphal tick from his upper arm on 3 September. The patient stored the tick in an empty vial at room temperature, and the tick was later identified as Amblyomma americanum. On 8 September, the patient began suffering from a per- sistent sore neck, characterized by musculoskeletal pain upon turning his head and insomnia due to pain. The pain was refractory to anti-inflammatory medications, including acetaminophen, aspirin and ibuprofen. Physi- cal examination on 23 September was unremarkable. Pyrexia was not observed and no erythema or edema was noted at the site of the tick bite; however, the patient had taken 500 mg aspirin prior to examination. The patient was treated for a presumptive tick-borne illness with 100 mg of oral doxycycline twice daily for 10 days. The patient reported that neck soreness was improved by 48 to 60 hours after doxycycline therapy was initiated. Laboratory testing Blood was drawn from the patient on 23 September for PCR testing for tick-borne diseases, on 26 September for a complete blood count (CBC) and acute serology, and on 15 October for convalescent serology. Whole blood from 23 September and sera from 26 September and 15 Octo- ber were submitted to the CDC for tick-borne disease test- ing. The CBC was performed by Quest Diagnostics (Nichols Institute, Chantilly, VA), and CBC results (Table 1) were within the normal reference range for this labora- tory. For PCR testing, DNA was extracted from 100 µl of clotted blood and from the dead tick, using an IsoQuick Nucleic Acid Extraction Kit (ORCA Research Inc., Bothell, WA). We detected DNA from Ehrlichia using a genus-specific, hemi-nested PCR with the outer primers EC12A and HE3 [4], followed by a hemi-nested reaction using the 'For- ward' primer [7] and HE3. DNA from Rickettsia species was detected using primer-1 and primer-2 [8]. We assessed the quality of the tick DNA using primers T1B and T2A [9]. Positive and negative controls were used for all assays and consisted of genomic DNA from Rickettsia rickettsii, Ehrlichia ewingii or distilled water. All PCR prod- ucts were purified with a QIAquick PCR Purification Kit (Qiagen, Valencia, CA) and sequenced in duplicate using PCR primers and a BigDye Terminator v3.1 Cycle Sequencing Kit (Applied Biosystems, Foster City, CA). Sequences were determined using an ABI 3100 (Applied Biosystems). Primer sequences were removed and sequences assembled with Seqmerge (Accelrys, San Diego, CA). Using the hemi-nested PCR, an amplicon from the 16S rRNA gene of an Ehrlichia species was obtained from the acute blood sample. The amplicon was sequenced, and the 361-bp sequence (GenBank accession number DQ217573 ) was 100% identical to the sequence reported from the Panola Mountain Ehrlichia species (Ehrlichia spe- cies P-Mtn, GenBank accession number DQ324367 ). The amplicon was not identical to sequences from any other species represented in GenBank. No DNA from Rickettsia was detected in the patient's blood. The tick was poorly preserved by the patient, and DNA could not be amplified from it. For acute and convalescent serology, sera from 26 Septem- ber and 15 October were tested using indirect immunoflu- orescence assays (IFA), performed as previously described [10], to detect antibodies against Anaplasma phagocy- tophilum, Borrelia burgdorferi, Coxiella burnetii, Francisella tularensis, Rickettsia africae, R. akari, 'R. amblyommii', R. conorii, R. parkeri, R. prowazekii, R. rickettsii and R. typhi, and antibodies cross-reactive with E. chaffeensis. We could not test the patient's serum against the Panola Mountain Ehrlichia species because this emerging agent has not yet been cultured. Antibody was detected using isotype-spe- cific goat antihuman immunoglobulin G (IgG) and human immunoglobulin M (IgM), labeled with fluores- cein isothiocyanate (FITC) (KPL, Gaithersburg, Mary- land). Prior to testing for IgM, sera were depleted of IgG Table 1: Complete blood count results for blood drawn on 26 September 2005 Hematocrit 46.7% Red blood cell count 5.32 × 10 7 /µl Hemoglobin 15.9 g/dl Mean corpuscular volume 87.8 fl Mean corpuscular hemoglobin 29.9 pg Mean corpuscular hemoglobin concentration 34.1 g/dl Red blood cell distribution width 12.7% Platelet count 272,000/µl White blood cell count 7500/µl Absolute neutrophils (%) 4868 cells/µl (64.9%) Absolute lymphocytes (%) 2243 cells/µl (29.9%) Absolute monocytes (%) 233 cells/µl (3.1%) Absolute eosinophils (%) 143 cells/µl (1.9%) Absolute basophils (%) 15 cells/µl (0.2%) Journal of Medical Case Reports 2008, 2:139 http://www.jmedicalcasereports.com/content/2/1/139 Page 3 of 3 (page number not for citation purposes) by use of a recombinant Protein G kit (Rapi-Sep-M, Pan- Bio, Columbia, MD). Acute and convalescent samples were tested side-by-side, and positive, negative and dilu- ent controls were assayed with the test samples and gave expected results. Serology did not support recent infection with any of the agents tested. With E. chaffeensis antigen, the patient's serum reacted with a small proportion of the organisms on the slide, as compared with positive control sera, and was considered cross-reactive in both acute and convalescent samples. Titers are expressed as the recipro- cal of the last dilution exhibiting specific fluorescence and were as follows: IgM 32 (26 September), and IgG 16 (26 September) and IgG 32 (15 October). Convalescent IgM data were not available. Conclusion We report that an emerging pathogen, the Panola Moun- tain Ehrlichia species, was detected in blood from a human patient following the bite of a nymphal Amblyo- mma that was probably acquired at Panola Mountain State Park in Georgia in the United States of America. The Panola Mountain Ehrlichia species was originally described from a goat fed upon by A. americanum col- lected at this park [4], but this is the first report associating the agent with human illness. The Panola Mountain Ehrlichia species is genetically closely related to E. ruminantium and more distantly related to E. chaffeensis [4]. The patient exhibited myalgia for 3 weeks prior to presentation, had ehrlichemia, which was confirmed by DNA sequencing at presentation, and rapidly recovered after treatment with doxycycline. Although PCR and serological testing for other tick-borne agents was negative, suggesting that ehrlichiosis was the cause of illness, we cannot conclusively rule out the possi- bility that the patient's symptoms were caused by an unknown factor. Serological confirmation of infection with the Panola Mountain Ehrlichia species could not be obtained, with only a two-fold rise in IgG titer between the two serum samples. This might be due to the initiation of antibiotic therapy prior to optimal immune response or due to the lack of an appropriate antigen; antibodies against ehrlichial agents are often, but not always, cross- reactive with other species of Ehrlichia [3]. In this case, PCR testing of whole blood was of significantly greater diagnostic value than serological testing. Abbreviations CBC: complete blood count; CDC: Centers for Disease Control; FITC: fluorescein isothiocyanate; IFA: immun- ofluorescence assays; IgG: immunoglobulin G; IgM: immunoglobulin M; PCR: polymerase chain reaction. Competing interests The authors declare that they have no competing interests. Authors' contributions WKR identified the tick, isolated DNA from the blood sample, performed sequencing reactions, analyzed data, and was a major contributor in writing the manuscript. ADL tested the DNA from the blood sample, recorded patient information, and was a major contributor in writ- ing the manuscript. WLN performed serological tests and reviewed drafts of this manuscript. AGC was the attending physician for the patient and contributed to drafts, collect- ing clinical specimens, and patient treatment and observa- tions. All authors read and approved the final manuscript. Consent Written informed consent was obtained from the patient for publication of this case report. A copy of the written consent is available for review by the Editor-in-Chief of this journal. Acknowledgements Diagnostic laboratory work was supported by the CDC and Department of Health and Human Services. The conclusions in this report do not nec- essarily represent the views of the funding agencies. We thank Gregory Dasch, Herbert Thompson, Robert Massung, Tonya Mixson and Martin Schreifer for their assistance. The use of trade names in this document does not constitute an official endorsement or approval of the use of such com- mercial hardware or software. References 1. Dumler JS, Madigan JE, Pusterla N, Bakken JS: Ehrlichioses in humans: epidemiology, clinical presentation, diagnosis, and treatment. Clin Infect Dis 2007, 45(Suppl 1):S45-S51. 2. Allsopp MTEP, Louw M, Meyer EC: Ehrlichia ruminantium – an emerging human pathogen. S Afr Med J 2005, 95:541. 3. Unver A, Perez M, Orellana N, Huang H, Rikihisa Y: Molecular and antigenic comparison of Ehrlichia canis isolates from dogs, ticks, and a human in Venezuela. J Clin Microbiol 2001, 39:2788-2793. 4. Loftis AD, Reeves WK, Spurlock JP, Mahan SM, Troughton DR, Dasch GA, Levin ML: Infection of a goat with a tick-transmitted Ehr- lichia from Georgia, U.S.A. that is closely related to Ehrlichia ruminantium. J Vector Ecol 2006, 31:213-223. 5. Case definitions for infectious conditions under public health surveillance: Ehrlichiosis, 2008 Case Definition [http:// www.cdc.gov/ncphi/disss/nndss/casedef/ehrlichiosis_2008.htm] 6. Prince LK, Shah AA, Martinez LJ, Moran KA: Ehrlichiosis: making the diagnosis in the acute setting. South Med J 2007, 100:825-828. 7. Li JS, Chu F, Reilly A, Winslow GM: Antibodies highly effective in SCID mice during infection by the intracellular bacterium Ehrlichia chaffeensis are of picomolar affinity and exhibit pref- erential epitope and isotype utilization. J Immunol 2002, 169:1419-1425. 8. Carl M, Tibbs CW, Dobson ME, Paparello S, Dasch GA: Diagnosis of acute typhus infection using the polymerase chain reac- tion. J Infect Dis 1990, 161:791-793. 9. Beati L, Keirans JE: Analysis of the systematic relationships among ticks of the genera Rhipicephalus and Boophilus (Acari: Ixodidae) based on mitochondrial 12S ribosomal DNA gene sequences and morphological characters. J Parasi- tol 2001, 87:32-48. 10. Nicholson WL, Comer JA, Sumner JW, Gingrich-Baker C, Coughlin RT, Magnarelli LA, Olson JG, Childs JE: An indirect immunofluo- rescence assay using a cell culture-derived antigen for detec- tion of antibodies to the agent of human granulocytic ehrlichiosis. J Clin Microbiol 1997, 35:1510-1516. . a human patient following the bite of a nymphal Amblyo- mma that was probably acquired at Panola Mountain State Park in Georgia in the United States of America. The Panola Mountain Ehrlichia species. We report here the first association of a recently discovered pathogen, the Panola Mountain Ehrlichia species, with a case of human illness. Case presentation: A 31-year-old man from Atlanta,. Central Page 1 of 3 (page number not for citation purposes) Journal of Medical Case Reports Open Access Case report The first report of human illness associated with the Panola Mountain Ehrlichia

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  • Abstract

    • Introduction

    • Case presentation

    • Conclusion

  • Introduction

  • Case presentation

  • Laboratory testing

  • Conclusion

  • Abbreviations

  • Competing interests

  • Authors' contributions

  • Consent

  • Acknowledgements

  • References

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